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Conditional protein degradation in using the auxin-inducible degron. | LitMetric

Conditional protein degradation in using the auxin-inducible degron.

Front Bioeng Biotechnol

Department of Molecular Biosciences and Bioengineering, University of Hawai'i at Manoa, Honolulu, HI, United States.

Published: May 2023

AI Article Synopsis

  • The auxin-inducible degron (AID) technology enables targeted protein degradation using a plant hormone, and this study showcases its application in an important oleaginous yeast.
  • Researchers successfully induced degradation of a superfolder GFP protein tagged with the mIAA7 degron by utilizing the OsTIR1 auxin receptor, though some unwanted degradation occurred without auxin.
  • The study also demonstrates the AID system's effectiveness in controlling the degradation of a metabolic enzyme involved in carotenoid production, reducing canthaxanthin output by about 50% when specific conditions were applied, highlighting areas for future development in improving this technique.

Article Abstract

Conditional protein degradation is a powerful tool for controlled protein knockdown. The auxin-inducible degron (AID) technology uses a plant auxin to induce depletion of degron-tagged proteins, and it has been shown to be functional in several non-plant eukaryotes. In this study, we demonstrated AID-based protein knockdown in an industrially important oleaginous yeast . Using the mini-IAA7 (mIAA7) degron derived from IAA7, coupled with an TIR1 (OsTIR1) plant auxin receptor F-box protein (expressed from the copper-inducible MT2 promoter), C-terminal degron-tagged superfolder GFP could be degraded in upon addition of copper and the synthetic auxin 1-Naphthaleneacetic acid (NAA). However, leaky degradation of the degron-tagged GFP in the absence of NAA was also noted. This NAA-independent degradation was largely eliminated by replacing the wild-type OsTIR1 and NAA with the OsTIR1 variant and the auxin derivative 5-Ad-IAA, respectively. Degradation of the degron-tagged GFP was rapid and efficient. However, Western blot analysis revealed cellular proteolytic cleavage within the mIAA7 degron sequence, leading to the production of a GFP sub-population lacking an intact degron. The utility of the mIAA7/OsTIR1 system was further explored in controlled degradation of a metabolic enzyme, β-carotene ketolase, which converts β-carotene to canthaxanthin via echinenone. This enzyme was tagged with the mIAA7 degron and expressed in a β-carotene producing strain that also expressed OsTIR1 controlled by the MT2 promoter. By adding copper and 5-Ad-IAA at the time of culture inoculation, canthaxanthin production was found to be reduced by about 50% on day five compared to the control culture without adding 5-Ad-IAA. This is the first report that demonstrates the efficacy of the AID system in . Further improvement of AID-based protein knockdown in may be achieved by preventing proteolytic removal of the mIAA7 degron tag.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC10264656PMC
http://dx.doi.org/10.3389/fbioe.2023.1188119DOI Listing

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